Fig. 5.
Fig. 5. Analysis of GAL4-CREB fusions by cotransfection assay. (A) Schematic structure of GAL4-CREB fusion constructs and reporter gene construct. (B) HEL cells were cotransfected with the pG4-CAT reporter gene and a gene encoding GAL4(1-147), GAL4-CREB▵LZ, or GAL4-CREB▵LZM1 and then treated with medium alone (negative control), TPO (100 ng/mL), Epo (2 U/mL), hemin (10−7 mol/L), forskolin (10−5 mol/L), or PMA (10−7 mol/L) for 30 minutes. CAT promoter activity was measured as folds of activations with respect to HEL cells left untreated (medium alone). Data are reported as the means ± SD of three independent transfection experiments performed in duplicate.

Analysis of GAL4-CREB fusions by cotransfection assay. (A) Schematic structure of GAL4-CREB fusion constructs and reporter gene construct. (B) HEL cells were cotransfected with the pG4-CAT reporter gene and a gene encoding GAL4(1-147), GAL4-CREB▵LZ, or GAL4-CREB▵LZM1 and then treated with medium alone (negative control), TPO (100 ng/mL), Epo (2 U/mL), hemin (10−7 mol/L), forskolin (10−5 mol/L), or PMA (10−7 mol/L) for 30 minutes. CAT promoter activity was measured as folds of activations with respect to HEL cells left untreated (medium alone). Data are reported as the means ± SD of three independent transfection experiments performed in duplicate.

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